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Cell Metabolic Alterations due to Mcph1 Mutation in Microcephaly

Cell Rep . 2020-04; 
NathalieJourniac,JavierGilabert-Juan,SaraCipriani,PauleBenit,XiaoqianLiu,SandrineJacquier,ValérieFaivre,AndréeDelahaye-Duriez,ZsoltCsaba,TristanHourcade,ElizaMelinte,SophieLebon,CélineViolle-Poirsier,Jean-FrançoisOury,HomaAdle-Biassette,Zhao-QiWang,ShyamalaMani,PierreRustin,JeannetteNardelli
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Gene Synthesis For transient expression in NPCs cells, the human full-length (FL) MCPH1 cDNA was synthesized with the HA-tag sequence fused at the 3′ end, and subcloned into the Xho/XbaI restriction sites of the pCAGGS-IRES-GFP (Addgene # 32482) plasmid by the customer service of the GenScript Biotech Corporation to generate the pCAGGS-MCPH1FL-HA. Get A Quote

摘要

A distinctive feature of neocortical development is the highly coordinated production of different progenitor cell subtypes, which are critical for ensuring adequate neurogenic outcome and the development of normal neocortical size. To further understand the mechanisms that underlie neocortical growth, we focused our studies on the microcephaly gene Mcph1, and we report here that Mcph1 (1) exerts its functions in rapidly dividing apical radial glial cells (aRGCs) during mouse neocortical development stages that precede indirect neurogenesis; (2) is expressed at mitochondria; and (3) controls the proper proliferation and survival of RGCs, potentially through crosstalk with cellular metabolic pathways involvin... More

关键词

VDAC1GRP75ATF4PCK2